Human desert hedgehog protein

ABSTRACT

Disclosed are a novel hedgehog protein, i.e., a Desert hedgehog protein of human origin including mature and precursor forms, a DNA encoding the protein, a monoclonal antibody recognizing the protein, a process for producing the protein, and a method for detecting the protein. The hedgehog protein is useful in establishment of hybridomas which produce antibodies recognizing the protein, and the monoclonal antibody is useful in detection and purification of the protein. The hedgehog protein, DNA, and monoclonal antibody of this invention have efficacy in elucidation of hereditary morphological abnormalities in humans to establish their treatments and diagnoses.

This is a division of copending parent application Ser. No. 09/063,778, filed Apr. 22, 1998.

BACKGROUND OF THE INVENTION

1. Field of the Invention

This invention relates to a novel hedgehog protein, more particularly, a Desert hedgehog protein of human origin.

2. Description of the Prior Art

The hedgehog gene was originally identified by genetic techniques as a gene that plays an important role in normal morphogenesis during embryonic and larval development in the fruit fly Drosophila melanogaster, as described by C. Nusslein-Volhard et al., in Nature, Vol.287, pp.795-801 (1980). J. J. Lee et al. sequenced the gene and deduced the amino acid sequence of the hedgehog protein as the expression product in Cell, Vol.71, pp.33-50 (1992). Some homologues of the gene were later isolated from vertebrates including mammals (hereinafter, the homologues of species other than the fruit fly may also be called “hedgehog”). At present, it is known that vertebrate hedgehog genes, unlike that of the fruit fly, form a multigene family and would play different roles in normal morphogenesis.

For example, as described by Y. Echelard et al., in Cell, Vol.75, pp.1417-1430 (1993), there have been identified three types of the genes of mouse origin, designated “Sonic hedgehog”, “Indian hedgehog”, and “Desert hedgehog”, which have different nucleotide sequences and express in different manners in living bodies. While in human, there have been found only two types of the genes designated “Sonic hedgehog” and “Indian hedgehog”, as described by V. Marigo et al., in GENOMICS, Vol.28, pp.44-51 (1995), and their expression manners and functions of their expression products remain to be elucidated. Therefore from scientific and pharmaceutical viewpoints, in order to elucidate the process of exhibiting hereditary morphological abnormalities in humans and direct research their treatments and diagnoses, the establishment of a novel hedgehog gene and its expression product, i.e. a novel hedgehog protein, is now in great expectation demand.

SUMMARY OF THE INVENTION

In view of the foregoing, the first object of this invention is to provide a novel hedgehog protein of human origin.

The second object of this invention is to provide a DNA encoding the hedgehog protein.

The third object of this invention is to provide a monoclonal antibody recognizing the hedgehog protein.

The fourth object of this invention is to provide a process for producing the hedgehog protein.

The fifth object of this invention is to provide a method for detecting the hedgehog protein.

The present inventors energetically and extensively screened for human cell lines which express a novel hedgehog gene capable of attaining the above objects by using RT-PCR techniques, where RNAs obtained from various established human cell lines were used as templates, while as primers various oligonucleotides were chemically synthesized based on the nucleotide sequence of mouse Desert hedgehog gene registered in “GenBank®”, a nucleic acid database by National Institute of Health, USA, under the accession number “X76292”. These screenings resulted in finding that some human cell lines including ARH-77 cell, ATCC CRL-1621, a cell line derived from plasma cell of a leukemia patient, expressed a specific gene in an elevated level checked with the above RT-PCRs. Further energetic studies confirmed that the human gene was a novel gene, which contained no known nucleotide sequences. Comparison with other genes revealed that the human gene has a relatively high homology to mouse Desert hedgehog gene. These findings led to the conclusion that the gene is a novel type of Desert hedgehog gene of human origin. A DNA obtained from the gene thus sequenced was introduced into Escherichia coli using an autonomously replicable vector, attaining satisfactory DNA expression and production of human Desert hedgehog protein.

Furthermore, the present inventors prepared known human Sonic hedgehog protein by using conventional recombinant DNA techniques and prepared monoclonal antibodies recognizing the protein. It was found that some of the monoclonal antibodies unexpectedly recognized well not only human Sonic hedgehog protein but also human Desert hedgehog protein. This invention was established based on these findings.

More particularly, the first object of this invention is attained by a Desert hedgehog protein of human origin.

The second object of this invention is attained by a DNA which encodes the hedgehog protein.

The third object of this invention is attained by a monoclonal antibody which recognizes the hedgehog protein.

The forth object of this invention is attained by a process for preparing a hedgehog protein which comprises the steps of allowing to express a DNA encoding the hedgehog protein and collecting the generated hedgehog protein.

The fifth object of this invention is attained by a method for detecting the hedgehog protein using a monoclonal antibody which recognizes the hedgehog protein.

BRIEF DESCRIPTION OF THE ACCOMPANYING DRAWINGS

FIG. 1 is the restriction map of the recombinant DNA of this invention “pHuDHH/pGEX-2T/#4-8”.

FIG. 2 is a half tone image of gel electrophoresis given on a display, visualized by Western blotting as the detection method using the monoclonal antibody of this invention.

FIG. 3 shows the results of detecting the hedgehog protein by an enzyme-immunoassay as the detection method using the monoclonal antibody of this invention.

In FIG. 1, the symbol “HuDHH” indicates a DNA encoding the hedgehog protein of this invention; the symbol “Amp”, an ampicillin-resistant gene; the symbol “pBR322ori”, a replication origin exerting in Escherichia coli; the symbol “GST”, a structural gene of glutathione S-transferase; and the symbol “Ptac”, a Tac promotor.

DETAILED DESCRIPTION OF THE INVENTION

This invention relates to a novel hedgehog protein, more particularly, a Desert hedgehog protein of human origin. The present hedgehog protein contains a part or the whole of the amino acid sequence of SEQ ID NO:1, which may bear a homology, usually about 80%, to mouse Desert hedgehog protein at amino acid sequence level. Examples of the present hedgehog protein are a mature form of human Desert hedgehog protein that contains the amino acid sequence of SEQ ID NO:1 and a precursor form of human Desert hedgehog protein that has the amino acid sequence of SEQ ID NO:2 or 3, which contains the amino acid sequence of SEQ ID NO:1. The present hedgehog protein further includes other types of proteins with amino acid sequences as illustrated above where one or more amino acids are deleted or replaced with other ones, one or more amino acids are added, or saccharide chains are linked, so far as they contain the amino acid sequence as mentioned above. The present hedgehog protein shall not be restricted to those obtained from specific sources and by specific preparation methods, threrefor it include natural proteins obtained from cultures of established cell lines, recombinant proteins obtained by recombinant DNA techniques, and synthetic polypeptides obtained by way of peptide synthesis.

The DNA of this invention includes any DNAs which encode such hedgehog protein, regardless of their sources or origins. Thus the DNA of this invention include those from natural sources as well as those artificially modified or chemically synthesized, as far as they encode the hedgehog protein of this invention. Generally in this field, in case of artificially expressing DNAs which encode proteins, one may replace one or more nucleotides in the DNAs with different nucleotides and/or link appropriate nucleotide sequences thereto with the purpose of improving their expression efficiency and/or the physiological and physicochemical properties of the protein. Such modification are feasible in the DNA of this invention. More particularly, one can link, for example, to the 5′- and/or 3′-termini of the DNA as described above, recognition sites for appropriate restriction enzymes, initiation codons, termination codons, promoters and/or enhancers, as far as the final protein products do retain prescribed properties. Thus, the wording “DNA” as referred to in this invention shall mean, in addition to those which encode the above-mentioned proteins, those which are complementary thereto, and those where one or more nucleotides have been replaced with different nucleotides while conserving the encoding amino acid sequence.

Such a DNA can be obtained from natural by screening of human cells, for example, mammalian cells including epithelial cells, endothelial cells, interstitial cells, chondrocytes, monocytes, granulocytes, lymphocytes, neurocytes, and established cell lines from them of human origin, based on a hybridization with a DNA as a probe which encodes at least a part of the amino acid sequence of human Desert hedgehog protein of this invention, for example, the amino acid sequence of SEQ ID NO:1. Such screening can be achieved with conventional methods commonly used in this field such as PCR, RT-PCR, screening cDNA libraries, screening genomic libraries and/or modified methods thereof. Examples of preferred cells are established cell lines including ARH-77 cell, ATCC CRL-1621, K-562 cell, ATCC CCL-243, and KU-812 cell, an cell line reported by K. Kishi, in Leukemia Research, Vol.9, pp.381-390 (1985), and bone mallow cells. The DNA of this invention thus obtained usually contains a part or the whole of the nucleotide sequence of SEQ ID NO:4. For example, from ARH-77 cell, ATCC CRL-1621, a DNA encoding a mature form of human Desert hedgehog protein that contains the nucleotide sequence of SEQ ID NO:4 or a DNA encoding a precursor form of human Desert hedgehog protein that has the nucleotide sequence of SEQ ID NO:5 or 6, which contains the nucleotide sequence of SEQ ID NO:4, can be obtained. The present DNA can also be obtained by conventional chemical synthesis. The DNA of this invention, once obtained in any manner, can be easily amplified to desired level by methods of PCR or those using autonomously replicable vectors.

The DNA of this invention includes those in the forms of recombinant DNAs where the DNA, encoding the present hedgehog protein, is inserted into autonomously replicable vectors. The recombinant DNAs can be relatively-easily obtained by using conventional recombinant DNA techniques, once the desired DNA is obtained. Examples of the vectors feasible in this invention are plasmid vectors including pGEX-2T, pGEX-4T-1, pKK223-3, pcDNAI/Amp, BCMGSNeo, pcDL-SRα, pKY4, pCDM8, pCEV4, and pME18S. The autonomously replicable vectors usually comprise nucleotide sequences suitable for the DNA expression in respective hosts, for example, promoters, enhancers, replication origins, terminators for transcription, splicing sequences, and/or sequences for selection markers. As the promotor, using a heat shock protein promotor or the interferon-α promotor disclosed in Japanese Patent Kokai No.163,368/95 by the same applicant makes it possible to regulate the present DNA expression in the transformants by external stimuli.

To insert the DNA of this invention, conventional methods comonly used in this field can be used. More particularly, a gene containing the DNA of this invention and an autonomously replicable vector are first cleaved with restriction enzymes and/or ultrasonication, then the resulting DNA and vector fragments are ligated. Ligation of the DNA and vector fragments become much easier when the genes and vectors are digested with restriction enzymes specific to particular nucleotides, for example, AccI, BamHI, BstXI, EcoRI, HindIII, NotI, PstI, SacI, SalI, SmaI, SpeI, XbaI and XhoI. To ligate the DNA and vector fragments, they can be first annealed, if necessary, and then exposed to DNA ligase in vivo or in vitro. The recombinant DNAs thus obtained are unlimitedly replicable in hosts of microbe and animal origins.

The DNA of this invention further includes those in the forms where the DNA, encoding the above-mentioned hedgehog protein, is introduced into desired hosts. The DNA in such forms can be obtained without considerable difficulty by introducing the recombinant DNA of this invention to desired hosts. For the hosts, cells of microbe, animal or plant origin conventionally used in this field can be arbitrarily used. The use of the hosts of microbe origin has a merit of a higher productivity of the protein per culture. The hosts of animal origin including mammals' has a merit that the protein produced is substantially or nearly equivalent to physicochemical properties of the protein obtained as a natural product. For the microbe hosts, for example, Escherichia coli, Bacillus species, Streptomyces species, and yeasts can be arbitrarily used. Examples of the mammalian hosts are epithelial cell, interstitial cell and hemopoietic cell of human, monkey, mouse and hamster origins including 3T3-Swiss albino cell, ATCC CCL-92, C127I cell, ATCC CRL-1616, CHO-K1 cell, ATCC CCL-61, CV-1 cell, ATCC CCL-70, COS-1 cell, ATCC CRL-1650, HeLa cell, ATCC CCL-2, MOP-8 cell, ATCC CRL1709, and their mutant strains. To introduce the DNA of this invention into such hosts, one can employ conventional methods, for example, DEAE-dextran method, calcium phosphate transfection method, electroporation method, lipofection method, microinjection method, and viral infection method using retrovirus, adenovirus, herpesvirus and vaccinia virus. To select clones capable of producing the protein among the resulting transformants, the transformants are cultivated in culture media, followed by selection of clones where production of the protein was observed. The above-mentioned recombinant DNA techniques are detailed in, for example, Jikken-Igaku-Bessatsu, Saibo-Kogaku Handbook (The handbook for the cell engineering), edited by Toshio KUROKI, Masaru TANIGUCHI and Mitsuo OSHIMURA, published by Yodosha. Co., Ltd., Tokyo, Japan (1992), and Jikken-Igaku-Bessatsu, Biomanual Series 3, Idenshi-Cloning-Jikken-Ho (The experimental methods for the gene cloning), edited by Takashi YOKOTA and Kenichi ARAI, published by Yodosha Co., Ltd., Tokyo, Japan (1993).

In this field, once a desired DNA is obtained as described above, then the DNA can be conventionally introduced into animals or plants to establish “transgenic animals” or “transgenic plants”. The transgenic animals and plants introduced with the DNA of this invention are also included by the DNA of this invention. The following outlines a procedure for establishing transgenic animals. At first, the DNA of this invention can be introduced into oosperms or embryonic stem cells by using microinjection method, electroporation method or infections with recombinant virus containing the DNA of this invention. Subsequently, thus-obtained cells introduced with the present DNA can be grafted into uterine tubes or uteruses of para-pregnant female animals. Thereafter, from the newborns delivered spontaneously or by caesarean, the transgenic animals introduced with the present DNA can be selected by hybridization method, PCR method, etc. The DNA to be introduced for the establishment of transgenic animals can comprise not only a nucleotide sequence for the present hedgehog protein but also other sequences for promotors or enhancers suitable for regulating the gene expression in desired tissue- and/or stimulation-specific manner and/or further other sequences for signal peptides. Thus, the transgenic animals introduced with the DNA of this invention can be obtained. Techniques for transgenic animals are detailed in a publication such as Jikken-Igaku-Bessatsu, Shin-Idenshikogaku-Handbook (The Handbook for Genetic Engineering), edited by Masami MURAMATSU, Hiroto OKAYAMA, and Tadashi Yamamoto, published by Yodosha Co., Ltd., Tokyo, Japan (1996), pp.269-283.

The present hedgehog protein can be prepared by the process of this invention comprising the steps of allowing to express a DNA encoding the hedgehog protein and collecting the generated hedgehog protein. The DNA expression step can include a step of culturing the above-mentioned transformants introduced with the DNA of this invention, encoding the hedgehog protein. The media used to culture the transformant can be selected from conventional ones depending on the types of the transformants to be used, and they are usually composed of, as a base, a bufferized water and, as additives, inorganic ions such as sodium ion, potassium ion, calcium ion, phosphoric ion and chloric ion; microelements, carbon sources, nitrogen sources, amino acids and vitamins which meet to the metabolism of particular hosts; and, optionally, sera, hormones, cell growth factors and cell adhesion factors. Examples of the carbon sources are saccharides including glucose, fructose, sucrose, starches, and partial hydrolyzates of starches, and examples of the nitrogen sources are nitrogen-containing inorganic and organic substances including ammonia, ammonium ions, urea, nitric ions, peptone, and yeast extracts.

Examples of the culture media are as follows: those for microbe hosts such as L broth medium, T broth medium, TY broth medium, nutrient broth medium, YM broth medium, and potato-dextrose medium; and those for animal hosts such as 199 medium, DMEM medium, Ham's F12 medium, IMDM medium, MCDB104 medium, MCDB153 medium, MEM medium, RD medium, RITC80-7 medium, RPMI-1630 medium, RPMI-1640 medium, WAJC404 medium. To the culture media, the transformant can be inoculated in a cell density of 1×10⁴-1×10⁷ cells/ml, preferably, 1×10⁵-1×10⁶ cells/ml, and cultured under conditions suitable for the hosts, if necessary, while the culture media are replaced with fresh preparations. In particular, when using the hosts of microbe origins, the culture can be carried out at a temperature of 25-65° C. and a pH of 5-8 under aerobic conditions such as agitation-aeration for 1-10 days. When using the hosts of animal origins, the culture can be carried out at a temperature of about 37° C. for one day to one week, preferably, two to four days by suspension- or monolayer culture. Thus cultures containing the present hedgehog protein are obtained. The content of the present hedgehog protein in the cultures, which may differ depending on the types of the transformants and culture conditions, is usually one microgram to 100 mg per liter.

Furthermore, in the process for preparing the hedgehog protein of this invention, the DNA expression step can include a step of culturing cells which express the hedgehog protein, for example, established human cell lines ARH-77 cell, ATCC CRL-1621, K-562 cell, ATCC CCL-243, and KU-812 cell, described by K. Kishi et al., in Leukemia Research, Vol.9, pp.381-390 (1985). By culturing such cells in culture media suitable for respective cells, for example, 199 medium, DMEM medium, Ham's F12 medium, IMDM medium, MCDB104 medium, MCDB153 medium, MEM medium, RD medium, RITC80-7 medium, RPMI-1630 medium, RPMI-1640 medium, and WAJC404 medium similarly as in culturing of the trasnformants using animal host cells as mentioned above, then the culture containing the present hedgehog protein can be obtained. The content of the present protein in the cultures, which may differ depending on the types of the cells and culture conditions, is usually one nanogram to one milligram per liter.

The culture products obtained in these manners can be first subjected to ultrasonication, cell-lytic enzyme and/or detergent to disrupt cells, if necessary, the present hedgehog protein can be separated from the cells or cell debris by filtration and centrifugation, followed by purification. In the purification, the culture products which have been separated from cells or cell debris can be subjected to conventional methods used to purify biologically-active proteins, for example, salting-out, dialysis, filtration, concentration, fractional precipitation, ion-exchange chromatography, gel filtration chromatography, adsorption chromatography, isoelectric focusing chromatography, hydrophobic chromatography, reversed phase chromatography, affinity chromatography, gel electrophoresis and isoelectric focusing gel electrophoresis which are used in combination, if necessary. The purified preparation of the present hedgehog protein can be concentrated and lyophilized into a liquid or solid form to meet to its final use. Immunoaffinity chromatographies using the monoclonal antibody described below do yield a high-purity preparation of the hedgehog protein with minimized costs and labors.

In the process of this invention for producing the hedgehog protein, the DNA expression step can also include a step of feeding or planting the transgenic animals or plants obtained by introducing the DNA which encodes the present hedgehog protein to animals other than humans or plants. After feeding or planting occasionally with desired stimuli, desired tissues, organs, bloods, milks, and/or body fluids of the resultants can be collected and subjected to the steps for purifying the hedgehog protein of this invention as mentioned above to obtain the present protein.

The monoclonal antibody of this invention includes the monoclonal antibodies in general which recognize the hedgehog protein of this invention, independently of its origins, sources, and classes. The monoclonal antibody of this invention can be obtained by using as an antigen the present hedgehog protein, other conventional hedgehog protein or antigenic fragment thereof, and more particularly, by preparing hybridoma cells of derived from an infinitely-proliferative of a mammal and an antibody-producing cell of a mammal that has been immunized with such an antigen, selecting clones of hybridoma capable of producing the monoclonal antibody of this invention, and culturing the clones in vitro or in vivo.

Proteins feasible as the antigens can be obtained through culturing of transformants introduced with a DNA encoding at least a partial amino acid sequence of SEQ ID NO:1, and the proteins are usually used after completely or partially purified. The antigenic fragments can be obtained by chemically or enzymatically digesting the completely or partially purified proteins or by chemical synthesis based on the amino acid sequence of SEQ ID NO:1, 2, or 3. Alternatively, the antigens can be obtained by using these techniques based on known hedgehog genes or proteins. Human Sonic hedgehog is useful as such known hedgehog.

Immunization of animals is conducted in conventional manner. For example, the antigens as described above can be injected alone or together with appropriate adjuvants into mammals through an intravenous, intradermal, subcutaneous or intraperitoneal route, and then the mammals can be fed for a prescribed time period. There is no limitation in types of the mammals, therefore any mammals can be used regardless of their types, sizes and genders, as far as one can obtain desired antigen-producing cells therefrom. Rodents such as rats, mice and hamsters are generally used, and among these the most desirable mammal can be chosen in respect to their compatibility with the infinitely-proliferative cells mentioned below. The dose of the antigen is generally set to about five to 500 μg/animal in total, which can be divided into two to five times inoculations with intervals of about one to two weeks, depending on the types and sizes of the mammals to be used. Three to five days after the final inoculation, the spleens are extracted and dispersed to obtain splenocytes as antibody-producing cells.

The antibody-producing cells obtained in this way can be then fused with infinitely-proliferative cells of mammalian origin to obtain cell-fusion products containing the objective hybridoma. Examples of the infinitely-proliferative cells usually used in this invention are cell lines of mouse myeloma origin such as P3/NSI/1-Ag4-1 cell, ATCC TIB-18; P3X63Ag8 cell, ATCC TIB-9; SP2/O-Ag14 cell, ATCC CRL-1581; and mutant strains thereof. The cell-fusion can be conducted in conventional manner using an electric pulse or a cell-fusion accelerator such as polyethylene glycol and Sendai virus. For example, the antibody-producing cells and the infinitely-proliferative cells of mammalian origin are co-suspended to give a ratio of about 1:1 to 1:10 in a cell fusion medium with such an accelerator and incubated at about 30 to 40° C. for about one to five minutes. Although conventional media such as minimum essential medium (MEM), RPMI-1640 medium, and Iscove's modified Dulbecco's medium are feasible as cell fusion media, it is desirable to remove the serum in media, such as bovine serum, prior to their use.

To select the objective hybridomas, the cell-fusion products thus obtained can be transferred to an appropriate selection medium, such as HAT medium, and the hybridomas are cultured at about 30 to 40° C. for 3 days to 3 weeks till the cells other than the hybridomas die. The hybridoma cells can be then cultured in usual manner and antibodies secreted in the medium can be tested for reactivity with the hedgehog protein of this invention. Such tests can be conducted in conventional manner directed to detection of antibodies in general, for example, enzyme-immunoassays, radioimmunoassays and bioassays, which are detailed in Tan-Clone-Kotai-Jikken-Manual (Experimental Manual for Monoclonal Antibody), edited by Sakuji TOYAMA and Tamie ANDO, published by Kodansha Scientific, Ltd., Tokyo, Japan (1991), pp.105-152. The hybridomas which recognize the present protein can be immediately cloned by the limiting dilution method, thus obtaining the singly cloned hybridomas according to this invention.

The monoclonal antibody of this invention can be obtained by culturing such hybridomas in vitro or in vivo. In culturing the hybridomas, conventional methods for culturing mammalian cells can be employed. More particularly, the monoclonal antibody can be collected from culture products in case of culturing in vitro in nutrient media, while the monoclonal antibody can be collected from the ascites and/or bloods of the animals in case of transplanting in non-human warm-blooded animals or culturing in vivo. To collect the monoclonal antibody from cultures, ascites and blood, conventional methods for purifying antibodies can be arbitrarily used. Particular methods are, for example, salting-out, dialysis, filtration, concentration, fractional precipitation, ion-exchange chromatography, gel filtration chromatography, adsorption chromatography, isoelectric focusing chromatography, hydrophobic chromatography, reversed phase chromatography, affinity chromatography, gel electrophoresis and isoelectric focusing gel electrophoresis which can be used in combination if necessary. The purified preparations of the monoclonal antibody can then be concentrated and dehydrated into liquids or solids to meet to their final use.

The monoclonal antibody of this invention is particularly useful in immunoaffinity chromatographies for purifying the present hedgehog protein. The method for purification usually comprises the steps of allowing the monoclonal antibody to contact with a mixture of the present protein and contaminants to adsorb the present hedgehog protein on the monoclonal antibody, and desorbing the protein from the antibody; these steps are usually conducted in aqueous systems. The monoclonal antibody of this invention can be used after being immobilized on gels of water-insoluble carriers and packed into columns. For example., the cultures of the transformants or their partially purified preparations are charged to such columns and run, resulting in that the hedgehog protein is substantially-selectively adsorbed by the monoclonal antibody on such carriers. The adsorbed protein can be easily desorbed by altering the hydrogen-ion concentration around the monoclonal antibody. For example, the desorption for eluting the protein is usually conducted under acidic conditions, preferably, pH 2-3 when using the monoclonal antibody belonging to immunoglobulin G (IgG), or alkaline conditions, preferably, pH 10-11 when using the monoclonal antibody belonging to immunoglobulin M (IgM). The present method can yield a high-purity preparation of the present hedgehog protein with minimized costs and labors.

The monoclonal antibody of this invention additionally has wide uses required to detect the present hedgehog protein. The use of the monoclonal antibody in label-immunoassays such as radioimmunoassays, enzyme-immunoassays, and fluorescent-immunoassays can make more rapidly and accurately detect the present hedgehog protein in samples qualitatively or quantitatively. In these immunoassays, the present monoclonal antibody can be used after being labelled with radioactive substances, enzymes, and/or fluorescent substances. The label-immunoassays have a merit that they can analyze more numerous samples at a time and more accurately than bioassays. Thus the detection method of this invention is significantly useful for quality controls of the present protein during processes of the production or the products, as well as for diagnoses of diseases by detecting the present hedgehog protein. This invention does not basically relate to the techniques for labelling monoclonal antibodies or label-assays, so that it does not describe them in detail. Such techniques are detailed in a publication such as Enzyme immunoassay, edited by P. Tijssen, translated by Eiji ISHIKAWA, published by Tokyo-Kagaku-Dojin, Tokyo, Japan (1989), pp.196-348.

The DNA of this invention, which encodes the present hedgehog protein, is also useful in “gene therapies”. Particularly, in usual gene therapies, the DNA of this invention can be first inserted into a vector derived from virus such as retrovirus, adenovirus or adeno-associated virus, alternatively, embedded in either cationic- or membrane fusible-liposomes. Subsequently, the inserted or embedded DNA can be directly injected into patients with the hedgehog protein susceptive diseases, alternatively, introduced in vitro into lymphocytes, which have been collected from the patients, and self-implanted to the patients. Thus, the DNA of this invention exhibits a remarkable efficacy in gene therapies for diseases being susceptive to human Desert hedgehog protein. General procedures for gene therapies are detailed in Jikken-Igaku-Bessatsu, Biomanual UP Series, Idenshichiryo-no-Kisogijutsu (Basic techniques for the gene therapy), edited by Takashi SHIMADA, Izumi SAITO, and Keiya OZAWA, published by Yodosha Co., Ltd., Tokyo, Japan (1996).

The following Examples describe in detail the way of practicing this invention. The hedgehog protein of this invention, the DNA encoding the hedgehog protein, and the process for producing the hedgehog protein are explained by Examples 1 to 3, the monoclonal antibody of this invention and process for preparing the antibody are explained by Example 4, and the method for detecting the hedgehog protein using the monoclonal antibody of this invention is explained by Examples 5 and 6. The following Examples can be diversified by the technical level in this field. In view of this, this invention should not be restricted to the Examples:

Example 1

Preparation of DNA

Example 1-1(a)

Preparation of Total RNA

ARH-77 cells, ATCC CRL-1621, an established cell line derived from human plasma cell leukemia, were suspended in RPMI1640 medium supplemented with 10%(v/v) fetal bovine serum and proliferated in usual manner at 37° C. in a 5%(v/v) CO₂ incubator while scaling up the culture. After the cell density reached a desired level, the cells were collected. The cells were suspended in micro-centrifugal tubes with phosphate-beffered saline (hereinafter, abbreviated as “PBS”) and centrifuged, and the supernatants were discarded; these treatments were repeated three times. Then the cells were placed in fresh micro-centrifugal tubes in an amount of 5×10⁶ cells/tube, and “ULTRASPEC™ RNA”, a total RNA isolation reagent commercialized by BIOTECX Laboratories, Inc., Houston, Tex., USA, was added to the tubes in a volume of 1.0 ml/tube before the cells were suspended. The suspensions were allowed to stand in ice-chilling conditions for 5 minutes, mixed with 1.2 ml/tube of a mixture of chloroform/“ULTRASPEC™ RNA” (⅕ by volume), shaken for 15 seconds, and allowed to stand in ice-chilling conditions for 5 minutes. Upper phase in the tubes formed by centrifugation was collected, mixed with the equal volume of 2-propanol, and allowed to stand in ice-chilling conditions for five minutes. The mixture was centrifuged, and the supernatant was discarded. The formed precipitate was washed twice with 75%(v/v) aqueous ethanol, dried up in vacuo, and dissolved in sterile distilled water, resulting in obtaining an aqueous solution containing total RNAs of ARH-77 cells. A small portion of the solution was examined for the absorbance at 260 nm to calculate an RNA content.

Example 1-1(b)

Preparation of First Strand cDNA

Based on the nucleotide sequence of a mouse Desert hedgehog gene registered in “GenBank® ”, a nucleic acid database by National Institute of Health, USA, under the accession number “X76292”, an oligonucleotide with the nucleotide sequence of 5′-GCCAGGGTGTGAGCAACAGT-3′ (SEQ ID NO:12) was prepared in usual manner. In a micro-reaction tube, 2.5 pmol of the oligonucleotide and one microgram of total RNAs prepared by the method in Example 1-1(a) were placed, and sterile distilled water was added to the mixture to give a final volume of 15.5 μl. After the tube was allowed to stand at 70° C. for ten minutes and under ice-chilling conditions for one minute, to the tube 2.5 μl of 10×PCR buffer, 2.5 μl of 25 mM MgCl2, 1.0 μl of 10 mM dNTP mix, and 2.5 μl of 0.1 M DTT were added in this order. The tube was allowed to stand at 42° C. for one minute. First strand cDNAs was synthesized by adding to the tube one microliter of “SUPERSCRIPT II RT”, a reagent of reverse transcriptase commercialized by GIBCO BRL, Life Technologies, Inc., Rockville, Md., USA, and incubating the tube at 42° C. for 50 minutes. After the mixture was heated to terminate the reaction at 70° C. for 15 minutes and cooled to 37° C., the RNAs were degraded by incubating with admixed one microliter of RNase at 37° C. for 30 minutes. Thereafter, from the reaction mixture, an aqueous solution containing purified first strand cDNAs in a volume of 50 μl was obtained by mixing with 120 μl of 6 M NaI and treating with “GlassMAX™”, a DNA isolation matrix commercialized by GIBCO BRL, Life Technologies, Inc., Rockville, Md., USA, in accordance with the accompanying instructions.

Example 1-1 (c)

Preparation of DNA Fragment Encoding the Hedgehog Protein and Recombinant DNA

Ten-microliter portion of a solution of first strand cDNAs, obtained by the method in Example 1-1 (b), was sampled in a micro-reaction tube and manipulated with “5′ RACE SYSTEM, VERSION 2.0”, a kit for a modified PCR method of 5′ RACE, commercialized by GIBCO BRL Life Technologies, Inc., Rockville, Md., USA, in accordance with the accompanying instructions to add a poly(C)-tail to each of the 5′-termini of the cDNAs and amplify DNA fragments for the 5′-terminal regions. The sense primer used was “anchor primer” in the kit, and the antisense primer used was the oligonucleotide in Example 1-1(b). The thermal controls were as follows: an incubation at 94° C. for one minute; 35 cycles of incubations at 94° C. for one minute, at 55° C. for one minute, and at 72° C. for one minute; and an incubation at 72° C. for 10 minutes. The reaction volume was set to 50 μl.

A DNA fragment which encodes a Desert hedgehog protein of human origin was obtained by PCR using the above reaction mixture as a template under conditions as follows. Sense and antisense primers for this PCR were obtained in usual manner based on the nucleotide sequence of a Desert hedgehog protein of mouse origin, which is reported by Y. Echelard et al. and registered in “GenBank®”, a nucleic acid database established by National Institute of Health, USA, under the accession number “x76292”; they had respective nucleotide sequences of 5′-TGTGCTGCTTGGCACTCTTG-3′ (SEQ ID NO:13) and 5′-CCGTGGCATTTCCCGGAAAG-3′ (SEQ ID NO:14). Two microliters of 100-folds dilution of the reaction mixture of the above 5′ RACE was placed in a fresh micro-reaction tube, then to which 3 μl of 10×PCR buffer, 1.8 μl of 25 mM MgCl₂, 0.6 μl of 10 mM dNTP mix, appropriate amounts of the sense and antisense primers, and sterile distilled water were added to give a final volume of 30 μl. After 0.3 μl of 5 units/μl Taq DNA polymerase was added to the tube, the mixture was subjected to an incubation at 94° C. for three minutes, 35 cycles of incubations at 94° C. for one minute, at 55° C. for one minute, and at 72° C. for one minute, and finally an incubation at 72° C. for 10 minutes, to effect PCR. The PCR products were subjected to 2%(w/v) agarose gel electrophoresis. A gel portion containing an about 600 bp-DNA band, stained with ethidium bromide, was excised and treated with “SUPREC™-01”, a DNA purification tube commercialized by Takara Shuzo Co., Ltd.,Tokyo, Japan, to obtain 20 μl aqueous solution containing a DNA fragment.

A portion of the DNA fragment solution was sampled and manipulated with “pCR—SCRIPT SK(+) CLONING KIT”, a DNA cloning kit commercialized by Stratagene Cloning Systems, California, USA, in accordance with the accompanying instructions to ligate the DNA fragment with “pCR-SCRIPT SK(+)”, the plasmid vector in the kit. After the ligation, a portion of the reaction mixture was introduced by conventional transformation method into competent cells of Escherichia coli “JM101” strain, commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, which were then inoculated on plates of L agar medium containing 50 μg/ml ampicillin and cultured at 37° C. under standing conditions overnight. Some of the colonies formed were respectively suspended in 10 μl aliquotes of sterile distilled water. PCRs were conducted under the same conditions as described above in this Example except for using the suspensions as respective templates. Colonies which gave an about 600 bp-DNA on agarose gel electrophoresis were respectively inoculated to aliquotes of L broth medium containing 50 μg/ml ampicillin and cultured at 37° C. under shaking conditions overnight. From the resulting cultures, recombinant DNAs were collected by conventional alkali-sodium dodecyl sulfate (hereinafter, sodium dodesyl sulfate is abbreviated as “SDS”) method. The recombinant DNAs were sequenced by dideoxy method. The DNA fragment in the recombinant DNAs contained the nucleotide sequence of SEQ ID NO:7.

Studying homology between thus-determined nucleotide sequence and other known nucleotide sequences, the nucleotide sequence determined in this Example exhibited a significant homology of about 89% to the nucleotide sequence of a mouse Desert hedgehog gene, registered in “GenBank®”, a nucleic acid database by National Institute of Health, USA, under the accession number “X76292”. This indicates that the DNA fragment of this Example encodes a human Desert hedgehog protein. The recombinant DNA obtained in this Example was named “pHuDHH/#20”. In addition, the nucleotide sequence of SEQ ID NO:7, determined in this Example, was compared with the informations on structures and functions of known hedgehog proteins as described by M. Hammerschmidt et al., in Trends in Genetics, Vol.13, pp.14-21 (1997), leading to a conclusion that the sequence of nucleotides 19-546 of SEQ ID NO:7 encodes a mature form of a human Desert hedgehog protein and that the mature form of the protein can contain the amino acid sequence shown along with this nucleotide sequence, which is also shown in SEQ ID NO:1.

Example 1-2

Preparation of DNA Fragment and Recombinant DNA Encoding the Hedgehog Protein

A recombinant DNA “pHuDHH/#20”, obtained by the method in Example 1-1(c), was cleaved with restriction enzymes EcoR1 and NotI and subjected to 2%(w/v) agarose gel electrophoresis. From the agarose gel, a gel portion containing an about 600 bp-DNA band stained with ethidium bromide was excised and treated with “SUPREC™-01”, a DNA purification tube commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, to collect and purify a DNA fragment. The purified DNA fragment was labelled with a radioisotope ³²P by using a DNA labelling kit, “MEGAPRIME™ DNA LABELLING SYSTEMS”, commercialized by Amersham Corp., Div. Amersham International, Arlington Heights, USA, and manipulating in accordance with the accompanying instructions. Human fetal brain cDNA library constructed with a type of bacteriophage λgtll as a vector, commercialized by CLONTECH Laboratories, Inc., Palo Alto, Calif., USA, was screened by using the ³²P-labelled DNA fragment as a probe. Cells of Escherichia coli strain “NM514” were infected with the cDNA library in usual manner, inoculated on plates of L agar medium, and cultured at 37° C. for 6-18 hours to form plaques. The formed plaques were transferred in usual manner to nylon membranes, which were then subjected to alkali-denaturalization, neutralization, and air-drying in usual manner. The air-dried membranes were immersed in a pre-hybridization solution, which contained 6×SSC, 5×Denhardt's solution, 0.5%(w/v) SDS, 50%(v/v) formamide, and 100 μg/ml denatured salmon sperm DNA, at 42° C. for 1-2 hours, and subsequently immersed in a fresh pre-hybridization solution with an appropriate amount of the ³²P-labelled DNA fragment added as a probe and incubated at 42° C. for 16-20 hours to effect hybridization. After the hybridization, the membranes were washed with 2×SSC containing 0.1%(w/v) SDS at ambient temperature for 15 minutes and further washed with 0.2×SSC containing 0.1%(w/v) SDS at a temperature moderately increasing from 37° C. to 65° C. until background radioactivity was adequately reduced. Thereafter the membranes were subjected to autoradiography. From a plaque which gave a positive signal, a phage clone was collected and amplified in usual manner, and from the amplified phage a DNA clone was collected. The DNA clone was sequenced by dideoxy method using primers prepared based on the vector's nucleotide sequence. The DNA clone contained a partial nucleotide sequence as shown with 5′-GTATCCATGGCTCTCCTG-3′ (SEQ ID NO:15). Compared with other known nucleotide sequences, the partial nucleotide sequence had a significant homology to a partial nucleotide sequence, containing translation initiation site, of a mouse Desert hedgehog gene registered in “GenBank®”, a nucleic acid database by National Institute of Health, USA, under the accession number “X76292”.

As sense and antisense primers for PCR, oligonucleotides with respective nucleotide sequences of 5′-GCCTCGAGGTATCCATGGCTCTCCTG-3′ (SEQ ID NO:16), which contains the above-determined partial nucleotide sequence, and 5′-GCGCGGCCGCTCAGCCGCCCGCCCGGAC-3′ (SEQ ID NO:17), which is complementary to the sequence of nucleotides 532-548 of SEQ ID NO:7, were prepared in usual manner. As a template one microliter portion of cDNAs solution, obtained by the methods in Examples 1-1(a) and 1-1(b), was placed in a micro-reaction tube, then to which 3 μl of 10×PCR buffer, 1.8 μl of 25 mM MgCl₂, 0.6 μl of 10 mM dNTP mix, appropriate amounts of the sense and antisense primers, and sterile distilled water were added to give a final volume of 30 μl. After 0.3 μl of 5 units/μl Taq DNA polymerase was added to thr tube, the mixture was subjected to an incubation at 94° C. for three minutes, 35 cycles of incubations at 94° C. for one minute, at 55° C. for one minute, and at 72° C. one minute, and finally an incubation at 72° C. for 10 minutes, to effect PCR. The PCR products were subjected to 2%(w/v) agarose gel electrophoresis. From the gel, a gel portion containing an about 600 bp-DNA band, stained with ethidium bromide, was excised and treated with “SUPREC™-01”, a DNA purification tube commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, to obtain 20 μl aqueous solution containing a DNA fragment.

A small portion of the DNA fragment solution was sampled and manipulated with “pT7BLUE CLONING KIT”, a DNA cloning kit commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, in accordance with the accompanying instructions to ligate the DNA fragment with “pT7BLUE”, the plasmid vecotor in the kit. After the ligation, a portion of the reaction mixture was introduced by usual transformation method into competent cells of Escherichia coli strain “JM101”, commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, which were then inoculated on plates of L agar medium containing 50 μg/ml ampicillin and cultured at 37° C. under standing conditions overnight. The formed colonies were respectively suspended in 10 μl aliquotes of sterile distilled water. Except for using the suspensions as respective templates, PCRs were conducted under the same conditions as in Example 1-1(c). Colonies which gave an about 600 bp-DNA band on agarose gel electrophoresis were respectively inoculated to aliquotes of L broth medium containing 50 μg/ml ampicillin and cultured at 37° C. under shaking conditions overnight. From the resulting cultures recombinant DNAs were collected by conventional alkali-SDS method. The recombinant DNAs were sequenced by dideoxy method. The DNA fragment in the recombinant DNAs contained the nucleotide sequence of SEQ ID NO:8, which can encode the amino acid sequence shown along with the nucleotide sequence.

The nucletotide sequence of SEQ ID NO:8 was compared with the nucleotide sequence of SEQ ID NO:7, determined in Example 1-1. The sequence of nucleotides 1-548 of SEQ ID NO:7 completely matched with the sequence of nucleotides 55-602 of SEQ ID NO:8. The results of this comparison and the comparison with the above-mentioned nucleotide sequence of a mouse Desert hedgehog gene revealed that: the nucleotide sequence of SEQ ID NO:8 encodes N-terminal region of a precursor form of a human Desert hedgehog protein; the sequence of nucleotides 7-72 of SEQ ID NO:8 encodes a signal peptide in a precursor form of the hedgehog protein; and the sequence of nucleotides 73-600 of SEQ ID NO:8 encodes a mature form of the hedgehog protein which contains the amino acid sequence of SEQ ID NO:1.

Example 1-3

Preparation of DNA Fragment and Recombinant DNA Encoding the Hedgehog Protein

As sense and antisense primers for PCR, oligonucleotides with respective nucleotide sequences of 5′-CGTGTCGGTCAAAGCTGATA-3′ (SEQ ID NO:18) and 5′-ATGCATTCCAGTCGGCTGGA-3′ (SEQ ID NO:19) were prepared in usual manner; the former sequence was identical to the sequence of nucleotides 501-520 of SEQ ID NO:7, and the latter sequence was based on the nucleotide sequence registered in “GenBank®”, a nucleic acid database by National Institute of Health, USA, under the accession number “AA064660”, which is of a human cDNA fragment similar to a 3′-terminal sequence for a mouse Desert hedgehog protein in a precursor form. As a template one microliter portion of cDNAs solution, obtained by the methods in Examples 1-1(a) and 1-1(b), was placed in a micro-reaction tube, then to which 3 μl of 10×PCR buffer, 1.8 μl of 25 mM MgCl₂, 0.6 μl of 10 mM dNTP mix, appropriate amounts of the above sense and antisense primers, and sterile distilled water were added to give a final volume of 30 μl. After 0.3 μl of 5 units/μl Taq DNA polymerase was added to the tube, the mixture was subjected to an incubation at 94° C. for three minutes, 35 cycles of incubations at 94° C. for one minute, at 55° C. for one minute, and at 72° C. one minute, and finally an incubation at 72° C. for 10 minutes to, effect PCR. The PCR products were subjected to 2%(w/v) agarose gel electrophoresis. From the gel, a gel potion containing an about 600 bp-DNA band, stained with ethidium bromide, was excised and treated with “SUPREC™-01”, a DNA purification tube commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, to obtain 20 μl aqueous solution containing a DNA fragment.

A portion of the DNA fragment solution was sampled and manipulated with “pT7BLUE CLONING KIT”, a DNA cloning kit commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, in accordance with the accompanying instructions to ligate the DNA fragment with “pT7BLUE”, the plasmid vector in the kit. After the ligation, a portion of the reaction mixture was introduced by usual transformation method into competent cells of Escherichia coli strain “JM101”, commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, which were then inoculated on plates of L agar medium containing 50 μg/ml ampicillin and cultured at 37° C. under standing conditions overnight. The formed colonies were respectively suspended in 10 μl aliquotes of sterile distilled water. Except for using the suspensions as respective templates and using the sense and antisense primers in this Example, PCRs were conducted under the same conditions as in Example 1-1(c). Colonies which gave an about 600 bp-DNA band on agarose gel electrophoresis were respectively inoculated to aliquotes of L broth medium containing 50 μg/ml ampicillin and cultured at 37° C. under shaking conditions overnight. From the resulting cultures recombinant DNAs were collected by conventional alkali-SDS method. The recombinant DNAs were sequenced by dideoxy method. The DNA fragment in the recombinant DNAs contained the nucleotide sequence of SEQ ID NO:9, which can encode the amino acid sequence shown along with the nucleotide sequence.

The nucleotide sequence of SEQ ID NO:9 was compared with the nucleotide sequence of SEQ ID NO:7, determined in Example 1-1. The sequence of nucleotides 501-548 of SEQ ID NO:7 completely matched with the sequence of nucleotides 1-48 of SEQ ID NO:9. In addition, the nucleotide sequence of SEQ ID NO:9 was compared with the informations on structure and function of known hedgehog proteins as described by M. Hammerschmidt et al., in Trends in Genetics, Vol.13, pp.14-21 (1997), revealing that the nucleotide sequence of SEQ ID NO:9 partially encodes a C-terminal region of a precursor form of a human Desert hedgehog protein.

Example 1-4

Preparation of DNA Fragment and Recombinant DNA Encoding the Hedgehog Protein

Total RNAs in a weight of 1.5 μg, obtained by the method in Example 1-1(a), was placed in a micro-reaction tube, to which 2 μl of 5×reverse transcriptase buffer, 2 μl of DTT, one microliter of 10 mM dNTP mix, an appropriate amount of an oligonucleotide as an adaptor primer for a modified PCR method of 3′ RACE with the nucleotide sequence of 5′-AAGGATCCGTCGACAAGCTTAATACGACGAATTCTGGAG(T)₁₇-3′ (SEQ ID NO:20) prepared in usual manner, and sterile distilled water were added to give a final volume of 29 μl. After admixed with one microliter of “SuperScript™ II RT”, a reagent of reverse transcriptase commercialized by GIBCO BRL Life Technologies Inc., Rockville, Md., USA, the tube was allowed to stand at 37° C. for about 1.5 hours to effect a reaction of synthesizing cDNAs to poly(A)*RNAs 3′-terminal regions. Except for using a portion of the reaction mixture as a template and oligonucleotides with respective nucleotide sequences of 5′-GGCTTCGACTGGGTCTACTA-3′ (SEQ ID NO:21) as a sense primer and 5′-AAGGATCCGTCGACAAG-3′ (SEQ ID NO:22) as an antisense primer prepared in usual manner, a first step PCR was conducted under the same conditions as in Example 1-3; the sequence of the sense primer was identical to the sequence of nucleotides 460-479 of SEQ ID NO:7, and that of the antisense primer was based on the above adaptor primer. After the first step PCR, the reaction mixture was diluted with an appropriate amount of sterile distilled water. Except for using the dilution as a template and oligonucleotides with the respective nucleotide sequences of 5′-ATGCGCTTCGGCCAGCG-3′ (SEQ ID NO:23) as a sense primer and 5′-GACAAGCTTAATACGAC-3′ (SEQ ID NO:24) as an antisense primer, a second step PCR was conducted under the same conditions as in Example 1-3; the sequence of the sense primer was identical to the sequence of nucleotides 369-385 of SEQ ID NO:9, and that of the antisense primer was based on the nucleotide sequence of the above adaptor primer. After the second step PCR, the reaction mixture was diluted with an appropriate amount of sterile distilled water. Except for using the dilution as a template and oligonucleotides with the respective nucleotide sequences of 5′-GTTCGCGCCGCTCACCG-3′ (SEQ ID NO:25) as a sense primer and 5′-TACGACGAATTCTGGAGT-3′ (SEQ ID NO:26) as an antisense primer, a third step PCR was conducted under the same conditions as in Example 1-3; the sequence of the sense primer was identical to the sequence of nucleotides 424-440 of SEQ ID NO:9, and that of the antisense primer was based on the nucleotide sequence of the above adaptor primer. The third step PCR products were subjected to 2%(w/v) agarose gel electrophoresis. From the gel, a gel portion containing an about 750 bp-DNA band stained with ethidium bromide was excised and treated with “SUPREC™-01”, a DNA purification tube commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, to obtain 20 μl aqueous solution containing a DNA fragment.

A portion of the DNA fragment solution was sampled and manipulated with “pT7BLUE CLONING KIT”, a DNA cloning kit commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, in accordance with the accompanying instructions to ligate the DNA fragment with “pT7BLUE”, the plasmid vector in the kit. After the ligation, a portion of the reaction mixture was introduced by usual transformation method into competent cells of Escherichia coli strain “JM101”, commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, which were then inoculated on plates of L agar medium containing 50 μg/ml ampicillin and cultured at 37° C. under standing conditions overnight. The formed colonies were respectively suspended in 10 μl aliquotes of sterile distilled water. Except for using the suspensions as respective templates and using the sense and antisense primers in the third step PCR, PCRs were conducted under the same conditions as in Example 1-1(c). Colonies which gave an about 750 bp-DNA band on agarose gel electrophoresis were respectively inoculated to aliquotes of L broth medium containing 50 μg/ml ampicillin and cultured at 37° C. under shaking conditions overnight. From the resulting cultures recombinant DNAs were collected by alkali-SDS method. The recombinant DNAs were sequenced by dideoxy method. The DNA fragment in the recombinant DNAs contained the nucleotide sequence of SEQ ID NO:10, which can encode the amino acid sequence shown along with the nucleotide sequence.

The nucleotide sequence of SEQ ID NO:10 was compared with the nucleotide sequence of SEQ ID NO:9, determined in Example 1-3. The sequence of nucleotides 1-152 of SEQ ID NO:10 completely matched with the sequence of nucleotides 424-575 of SEQ ID NO:9. The results of this comparison and the comparison with the above-mentioned nucleotide sequence of a mouse Desert hedgehog gene revealed that the nucleotide sequence of SEQ ID NO:10 encodes a region containing the C-terminus of a precursor form of a human Desert hedgehog protein.

As described in Examples 1-1 to 1-4, the nucleotide sequences of SEQ ID NOs:7-10, determined in these Examples, were proved to be overlapping nucleotide sequences one another which partially encode a precursor form of a human Desert hedgehog protein; and the precursor protein can be wholly encoded by a DNA containing the nucleotide sequence of SEQ ID NO:6. In addition, these results elucidated that: a human Desert hedgehog protein can be in a precursor form which contains the amino acid sequence of SEQ ID NO:2 or 3 or in a mature form which contains the amino acid sequence of SEQ ID NO:1; such precursor protein can be encoded by a DNA containing the nucleotide sequence of SEQ ID NO:5 or 6, respectively; and such mature protein can be encoded by a DNA containing the nucleotide sequence of SEQ ID NO:4.

Example 2

Preparation of Transformant

Based on the nucleotide sequence determined in Example 1-1(c), which encodes a precursor form of a human Desert hedgehog protein, oligonucleotides with respective nucleotide sequences of 5′-CCCGGGAATTCATTGCGGGCCGGGCCGGGGGCCG-3′ (SEQ ID NO:27) as a sense primer and 5′-ACGATGAATTCTCAGCCGCCCGCCCGGACCGCCA-3′ (SEQ ID NO:28) as an antisense primer were prepared in usual manner. PCR was conducted under the same conditions as in Example 1-1(c) except for using the recombinant DNA “pHuDHH/#20” as a template, obtained by the method in Example 1-1(c), and the above sense and antisense primers. An about 600 bp-DNA amplified in this PCR was purified by 2%(w/v) agarose gel electrophoresis and treating with “SUPREC™-01”, a DNA purification tube commercialized by Takara Shuzo Co., Ltd., Tokyo, Japan, in accordance with the accompanying instruction, to obtain 20 μl aqueous DNA solution. Two microliters portion of the DNA solution was sampled and subjected to a ligation reaction using T4 DNA ligase with “pCR™II”, a plasmid vector for TA cloning commercialized by Invitrogen Corporation, San Diego, USA. A portion of the reaction mixture was introduced by usual transformation method into competent cells of Escherichia coli strain “TOP10F'”, commercialized by Invitrogen Corporation, San Diego, USA, which were then inoculated on plates of L agar medium containing 50 μg/ml ampicillin and 50 μg/ml 5-bromo-4-chrolo-3-indolyl-β-D-galactoside and cultured at 37° C. under standing conditions. A white colony formed was inoculated to an aliquote of L broth medium containing 50 μg/ml ampicillin and cultured at 37° C. under shaking conditions overnight. From the resulting culture, a recombinant DNA was collected by alkali-SDS method. The recombinant DNA was treated with restriction enzyme EcoRI and subjected to 2%(w/v) agarose gel electrophoresis, on which an about 600 bp-DNA was separated, and it was then purified with “SUPREC™-01”, a DNA purification tube commercialized by Takara Shuzo Co., Ltd, Tokyo, Japan.

A portion of the purified DNA solution was sampled and subjected to a ligation reaction in usual manner using T4 DNA ligase with plasmid vector “pGEX-2T”, commercialized by Pharmacia Biotech, Inc., Uppsala, Sweden, which had been cleaved with EcoRI and dephosphorylated prior to use. A portion of the ligation reaction mixture was introduced by usual transformation method into competent cells prepared by applying the method in DNA cloning, Vol.1, edited by D. M. Glover, published by IRL press limited, Oxford, England (1985), pp.109-136, to Escherichia coli “BL21” strain, commercialized by Pharmacia Biotech, Inc., Uppsala, Sweden, which were then inoculated to plates of L agar medium containing 50 μg/ml ampicillin and cultured at 37° C. under standing conditions overnight. A colony formed was inoculated to an aliquote of L both medium containing 50 μg/ml ampicillin and cultured at 37° C. under shaking conditions overnight. From the resulting culture, a recombinant DNA was collected by alkali-SDS method. The recombinant DNA was confirmed by dideoxy method to contain the nucleotide sequence of SEQ ID NO:4, encoding the amino acid sequence of SEQ ID NO:1. The recombinant DNA and the transformant with the recombinant DNA introduced, thus obtained, were named “pHuDHH5′/pGEX-2T/#4-8” and “TAL#4-8/HuDHH”, respectively. As shown in FIG. 1, in the recombinant DNA “pHuDHH5′/pGEX-2T/#4-8”, the DNA with the nucleotide sequence of SEQ ID NO:4 encoding a mature form of a human Desert hedgehog protein and a termination codon were respectively located in the downstream and further downstream of a structural gene of glutathione S-transferase in the same frame with the gene, which was under the regulation of Tac promotor.

Example 3

Production of the hedgehog protein A transformant “TAL#4-8/HuDHH” obtained by the method in Example 2 was cultured in L broth medium containing 50 μg/ml ampicillin at 37° C. under shaking conditions overnight to obtain a seed culture. One milliliter of the seed culture was added to 100 ml of the same medium, freshly prepared in a 500 ml-Erlenmeyer flask, and cultured at 37° C. under shaking conditions while the absorbance at 600 nm was monitored. When the absorbance reached a value of 0.5, 0.1 ml of 100 mM isopropylthio-β-D-galactoside was added to the culture. After further cultivation at 37° C. for 3.5 hours, the cells were collected from the culture by centrifugation. The cells were washed with PBS, suspended in 5 ml of fresh preparation of PBS, and disrupted with ultrasonication in usual manner. After the cell-disruptant was centrifuged, the formed supernatant was collected.

The supernatant was added to “GLUTATHIONE SEPHAROSE 4B BEADS”, a preparation of sepharose beads linked to glutathione, commercialized by Pharmacia Biotech, Inc., Uppsala, Sweden, and incubated at ambient temperature for 30 minutes. After centrifugation of the mixture and discard of the resulting supernatant, the beads were washed twice with PBS. To the beads, an appropriate amount of 50 mM Tris-HCl buffer (pH 7.5) containing 2.5 mM CaCl₂ and 150 mM NaCl was added, and admixed with 10 units of thrombin, commercialized by Ito Ham Co., Ltd., Nishinomiya, Japan, per one milligram of the proteinaceous components. The mixture was incubated at ambient temperature for 16 hours. The mixture was centrifuged to collect a supernatant, which was then admixed with an appropriate amount of “ANTITHROMBIN AGAROSE”, commercialized by Sigma Chemical Company, St. Louis, Mo., USA, and centrifuged. The resulting supernatant was added to “HEPARIN AGAROSE”, commercialized by Sigma Chemical Company, St. Louis, Mo., USA, previously equilibrated with equilibration buffer (PBS containing 1.0 mM DTT and 0.2 mM phenylmethanesulfonyl fluoride), and incubated at ambient temperature for 30 minutes. The mixture was admixed with an appropriate amount of equilibration buffer and centrifuged, and the resulting supernatant was discarded. To the remaining components an appropriate amount of 650 mM NaCl was added, and the resulting mixture was centrifuged to collect a supernatant. These treatments, i.e., addition of 650 mM NaCl, centrifugation, and collection of a supernatant, were additionally applied twice to the remaining components, and the supernatants thus obtained were pooled.

A portion of the pooled liquid was subjected to SDS-polyacrylamide gel electrophoresis (hereinafter, abbreviated as “SDS-PAGE”) in the presence of a reducing agent, in accordance with the method by U. K. Laemli, in Nature, Vol.227, pp.680-685 (1970). As molecular weight markers “SDS-PAGE STANDARDS, LOW RANGE”, containing six proteins with distinctive molecular weights of 14,400-97,400 daltons, commercialized by Bio-rad Laboratories Inc., Richmond, USA, was used. Main bands were observed at positions corresponding to molecular weights of about 22,000±2,000 daltons and about 18,000±2,000 daltons. Reference 1 was conducted in the same manner as in this Example except for using Escherichia coli “BL21” strain in place of the transformant “TAL#4-8/HuDHH”, giving no remarkable band on SDS-PAGE. Reference 2 was conducted in the same manner as this Example except for using Escherichia coli “BL21” strain transformed with the plasmid vector “pGEX-2T” in place of the transformant “TAL#4-8/HuDHH”, giving no remarkable band on SDS-PAGE.

The molecular weight of a human Desert hedgehog protein in a mature form which has the amino acid sequence of SEQ ID NO:1 is calculated to be 19,747. According to this Example, the objective protein is usually generated in a form with a peptide as shown by Gly-Ser-Pro-Gly-Ile-His- (SEQ ID NO:29) added to the N-terminus and collected. The molecular weight of a protein that has the amino acid sequence of SEQ ID NO:1 and Gly-Ser-Pro-Glylle-His-(SEQ ID NO:29), which is added to the N-terminus of SEQ ID NO:1, is calculated to be 20,296. These indicate that the protein obtained by the method in this Example which gave a molecular weight of 22,000±2,000 daltons on SDS-PAGE is a type of the present hedgehog protein, containing the amino acid sequence of SEQ ID NO:1. The other protein obtained by the method in this Example, which gave a molecular weight of 18,000±2,000 daltons on SDS-PAGE, is considered to be a degradation product of the hedgehog protein formed during the process of this Example. These results mean that the process of this invention satisfactorily produces a human Desert hedgehog protein of this invention.

Example 4

Production of Monoclonal Antibody

Example 4-1

Preparation of Immunogen

Example 4-1(a)

Preparation of Transformant Introduced with DNA that Encodes Immunogen

A549 cells, ATCC CCL-185, an established cell line derived from a human lung carcinoma, were suspended in RPMI-1640 medium (pH 7.2) supplemented with 10%(v/v) fetal bovine serum and proliferated in usual manner at 37° C. in a 5%(v/v) CO₂ incubator while scaling up the culture. After the cell density reached a desired level, proliferated cells were collected. The cells were manipulated with “ULTRASPEC™ RNA”, similarly as in Example 1-1(a), to obtain an aqueous solution containing total RNAs of A549 cells. By applying usual RT-PCR method to the total RNAs, a DNA fragment encoding a mature form of a human Sonic hedgehog protein was amplified. As the sense and antisense primers in this RTPCR, oligonucleotides with respective nucleotide sequences of 5′CCCGGGAATTCATTGCGGACCGGGCAGGGGGTT-3′ (SEQ ID NO:30) and 5′ACGATGAATTCTCAGCCTCCCGATTTGGCCGC-3′ (SEQ ID NO:31), prepared in usual manner based on the nucleotide sequence of a human Sonic hedgehog gene, reported by V. Marigo et al. and registered in “GenBank®”, a nucleic acid database by National Institute of Health, USA, under the accession number “L38518”, were used. The amplified DNA fragment was collected by treating the RT-PCR products with “SUPREC™-01”, as in Example 1-1(c). Similarly as in Example 1-1(c), the DNA fragment was ligated with plasmid vector “PCRIII” and introduced into Escherichia coli “TOP10F′” strain, the obtained transformant was cultured, and from the resulting culture a recombinant DNA was collected by alkali-SDS method. The recombinant DNA was sequenced by dideoxy method, confirming that it contained the nucleotide sequence of SEQ ID NO:11, encoding a human Sonic hedgehog protein in a mature form.

Similarly as in Example 2, an aliquot of the recombinant DNA was cleaved with restriction enzyme EcoRI to form an about 600 bp-DNA, which was then collected by treating with “SUPREC™-01”, ligated with plasmid vector “pGEX-2T”, and introduced into Escherichia coli “BL21” strain. The obtained transformant was cultured, and from the resulting culture a recombinant DNA was collected by alkali-SDS method. The recombinant DNA was sequenced by dideoxy method, confirming that it contained a DNA with the nucleotide sequence of SEQ ID NO:11 and a termination codon, which are respectively located in the downstream and further downstream of a structural gene of glutathione S-transferase in the same frame under the regulation of Tac promotor. The recombinant DNA and the transformant with the recombinant DNA introduced, thus obtained, were named “pHuSHH/pGEX-2T/#3-1” and “TAL#3-1/HuSHH”, respectively.

Example 4-1(b)

Preparation of Immunogen using Transformant

Similarly as in Example 3, the transformant “TAL#3-1/HuSHH” obtained by the method in Example 4-1(a) was cultured, the proliferated cells were collected from the culture, and a supernatant of the cell-disruptant was obtained. By applying the methods using “GLUTATHIONE SEPHAROSE 4B BEADS”, thrombin, “ANTITHROMBIN AGAROSE” and “HEPARIN AGAROSE” in Example 3 to the supernatant, an aqueous solution containing a protein derived from “TAL#3-1/HuSHH” was obtained, and analyzed by SDS-PAGE; a main band was observed at a position corresponding to a molecular weight of 22,000±2,000. The molecular weight of a mature form of a human Sonic hedgehog protein which has the amino acid sequence shown along with SEQ ID NO:11 is calculated to be 19,747. According to this Example, the objective protein is usually generated in a form with a peptide as shown by Gly-SerPro-Gly-Ile-His-(SEQ ID NO:29) added to the N-terminus and collected. These indicate that the protein obtained in this Example is a human Sonic hedgehog protein with a satisfactory purity. Thus, a purified preparation of a human Sonic hedgehog protein as an immunogen was obtained.

Example 4-2

Preparation of Hybridoma

Seven-week-old BALB/c mice were intraperinoneally injected with a purified preparation of a human Sonic hedgehog protein, obtained by the method in Example 4-1(b), in a dose of 100 μg/body together with complete Freund adjuvant in usual manner. Two weeks later, the above injection was repeated, and then the mice were injected with incomplete Freund adjuvant three times with one-week interval. On the fourth day after the final injection, spleens were extracted from the mice and dispersed to obtain splenocytes.

The splenocytes and SP2/0-Ag14 cells, ATCC CRL-1581, derived from mouse, were co-suspended in a serum-free RPMI 1640 medium, which had been warmed prior to use to 37° C., to give respective cell densities of 3×10⁴ and 1×10⁴ cells/ml, and then centrifuged to collect a precipitate. To the precipitate, one milliliter of a serum-free RPMI 1640 medium (pH 7.2) containing 50%(w/v) polyethylene glycol with an average molecular weight of about 15,000 daltons was dropped over one minute, and the resulting mixture was incubated at 37° C. for one minute. A serumfree RPMI 1640 medium (pH 7.2) was further dropped to the mixture to give a final volume of 50 ml, which was then centrifuged to collect a precipitate. The precipitate was suspended in HAT medium, distributed to wells of 96-well microplates in a volume of 200 μl/well, and incubated at 37° C. for a week to select hybridomas.

Antibodies secreted in culture supernatants in the wells were tested for a reactivity with a Sonic hedgehog protein, obtained in Example 4-1(b), by conventional enzyme-immunoassay to select hybridomas which exhibited the reactivity. The antibodies secreted in the culture supernatants of the selected hybridomas were further tested for another reactivity with the hedgehog protein of this invention, obtained in Example 3, by conventional enzyme-immunoassay to select hybridomas which additionally exhibited the reactively. Thereafter, the finally selected hybridomas were repeatedly subjected to limiting dilution method, resulting in obtaining hybridoma clones capable of producing the monoclonal antibody of this invention which were named “SH2-3”, “SH2-21”, and “SH2-260”.

Example 4-3

Production of Monoclonal Antibody

Hybridomas “SH2-3”, “SH2-21”, and “SH2-260” obtained in Example 4-2 were separately suspended to give a cell density of 1×10⁶ cells/ml each in aliquotes of RPMI 1640 medium (pH 7.2) supplemented with 5%(v/v) fetal bovine serum, and cultured at 37° C. in a 5%(v/v) CO₂ incubator while scaling up the culture. After the cell densities reached a desired level, the hybridomas were peritoneally injected in a dose of 1×10⁷ cells/body to eight-week-old BALB/c mice which had been peritoneally injected with 0.5 ml/body “PRISTANE”, a reagent of 2,6,10,14-tetramethylpentadecane commercialized by Aldrich Chemical Co., Inc., Milwaukee, USA, and the mice were fed for a week in usual manner.

From the respective lines of mice, ascites were collected and threefold diluted with PBS. To the dilutions, ammonium sulfate was added to give 50% saturation. The resulting mixture was allowed to stand at 4° C. for 24 hours and then centrifuged to collect precipitates. The precipitates were dialyzed against 20 mM KH₂PO₄ (pH 6.7) at 4° C. overnight, and then charged to columns of hydroxyapatite, pre-equilibrated with 20 mM KH₂PO₄ (pH 6.7). Through the columns, running KH₂PO₄ (pH 6.7) solution with increasing concentration from 20 to 300 mM in a linear gradient manner resulted in obtaining aqueous solutions of “SH2-3 mAb”, “SH2-21 mAb”, and “SH2-260 mAb”, the monoclonal antibodies of this invention. The yields were about 5 mg/mouse each. Analyzing in usual manner, all of the monoclonal antibodies belonged to a class of IgG₁.

Example 5

Western Blotting

One microgram of a Desert hedgehog protein, obtained by the method in Example 3, was subjected to SDS-PAGE with 15%(w/v) gel in the presence of a reducing agent. In parallel, 50 ng of a Sonic hedgehog protein, obtained by the method in Example 4-1(b), was subjected to SDS-PAGE with 13%(w/v) gel in the presence of a reducing agent. In usual manner, proteinaceous components in the gels were transferred to nitrocellulose membranes, which were then immersed in “BLOCK ACES™”, an immobilizing agent commercialized by Dainippon Pharmaceutical Co., Ltd., Osaka, Japan, to effect blocking. The membranes were immersed in PBS containing 20 μg/ml “SH2-3 mAb”, monoclonal antibody obtained by the method in Example 4-3, 10%(v/v) “BLOCK ACE™, and 0.1%(v/v) “TWEEN20”, a detergent commercialized by City Chemical Corp., New York, U.S.A., for one hour; and washed with PBS containing 0.1%(v/v) “TWEEN 20” to remove excessive antibodies. Thereafter, the nitrocellulose membranes were reacted for one hour in PBS containing 0.1%(v/v) sheep anti-mouse immunoglobulin antibody labelled with horseradish peroxidase, 10%(v/v) “BLOCK ACE™”, and 0.05%(v/v) “TWEEN 20”; washed with PBS containing 0.1%(v/v) “TWEEN 20”; and color-developed by using “ECL™ KIT”, a kit for color development commercialized by Amersham International plc, Buckinghamshire, UK. The molecular weight markers used were “SDS-PAGE STANDARDS, LOW RANGE”, containing six proteins having distinctive molecular weights of 14,400-97,400 daltons, commercialized by Bio-rad Laboratories Inc., Richmond, USA. The results are in FIG. 2.

In FIG. 2, on Lane 1, the band corresponding to a molecular weight of 22,000±2,000 is of the hedgehog protein of this invention, and the other band, corresponding to a molecular weight of 18,000±2,000, is of the degradation product of the hedgehog protein formed during the process in Example 3. In FIG. 2, on Lane 2, the band corresponding to a molecular weight of 22,000±2,000 is of a human Sonic hedgehog protein, obtained by the method in Example 4-1(b).

Another Western blotting which was conducted in the same manner as above except for using a monoclonal antibody “SH2-21 mAb”, obtained by the method in Example 4-3, in place of the monoclonal antibody “SH2-3 mAb”, giving similar results as above. These results indicate that the monoclonal antibodies, according to this invention, well recognized not only a human Sonic hedgehog protein but also a human Desert hedgehog protein.

Example 6

Enzyme-Immunoassay

Monoclonal antibodies “SH2-3 mAb” and “SH2-260 mAb”, obtained by the method in Example 4-3, were co-diluted in PBS to give a concentration of 10 μg/ml each, the resulting solution was distributed to wells of 96-well microplates in a volume of 100 μl/well. The microplates were incubated at ambient temperature. From the microplates the solution was removed, and PBS containing 1%(w/v) bovine serum albumin was distributed to the wells in a volume of 200 μl/well. Then the microplates were allowed to stand at 4° C. overnight. In parallel, a human Desert hedgehog protein, obtained by the method in Example 3, and a human Sonic hedgehog protein, obtained by the method in Example 4-1(b), were separately diluted with PBS to give desired different concentrations. After removing the solution from the microplates, and the respective hedgehog protein solutions were added to the wells and reacted at ambient temperature for one hour. The microplates were washed with PBS containing 0.05%(v/v) “TWEEN 20”, and added with a rabbit anti-hedgehog protein antiserum 500-fold diluted with PBS in a volume of 100 μl/well. The antiserum used in this Example was obtained by immunizing rabbits with a human Sonic hedgehog protein, obtained by the method in Example 4-1(b), and collecting serum from the rabbits in usual manner.

After the reaction with the antiserum, the microplates were washed with PBS containing 0.05%(v/v) “TWEEN 20” and added with a horseradish peroxidase-labelled donkey anti-rabbit immunoglobulin antibody, commercialized by Amersham International plc, Buckinghamshire, UK, which had been 1000-fold diluted with PBS, followed by allowing the microplates to stand at ambient temperature for one hour. The microplates were washed with PBS containing 0.05%(v/v) “TWEEN 20”. Thereafter, in usual manner, a mixture solution of o-phenylene diamine as a substrate and H₂O₂ was added to the wells in a volume of 100 μl/well followed by an incubation at ambient temperature for 15 minutes to effect enzyme reaction, and the reaction was terminated by 2N H₂SO₄ added. Intensities of colors in the wells developed by the reaction were estimated by measuring the absorbance at 492 nm. The results are in FIG. 3.

The results in FIG. 3. indicate that the method for detecting, according to this invention, well detected not only a human Sonic hedgehog protein but also a human Desert hedgehog protein.

As described above, this invention was established based on the finding of a novel hedgehog protein, i.e., a Desert hedgehog protein of human origin. The hedgehog protein of this invention is useful in establishment of a hybridoma capable of producing a monoclonal antibody that recognizes the protein. The hedgehog protein of this invention has efficacy in treatment and prevention of susceptive diseases to the hedgehog protein. The monoclonal antibody is useful in purification and detection of human Desert hedgehog protein because the antibody recognizes the hedgehog protein. The monoclonal antibody has efficacy in treatment, prevention, and diagnosis of diseases relating to excessive production of the hedgehog protein in living bodies. In addition to these effectiveness, the protein, DNA, and monoclonal antibody of this invention are extremely useful in elucidation of the process of exhibiting hereditary morphological abnormalities in humans. The process of this invention does satisfactorily produce the hedgehog protein.

This invention, which exhibits these remarkable effects, would be very significant and contributive to the art.

While there has been described what is at present considered to be the preferred embodiments of the present invention, it will be understood the various modifications may be made therein, and it is intended to cover in the appended claims all such modifications as fall within the true spirits and scope of the invention. 

1. An isolated DNA which encodes a desert hedgehog protein of human origin having the amino acid sequence of SEQ ID NO:1, or an isolated DNA complementary thereto.
 2. An isolated DNA which encodes a desert hedgehog protein of human origin having the amino acid sequence of SEQ ID NO:2, or an isolated DNA complementary thereto.
 3. An isolated DNA which encodes a desert hedgehog protein of human origin having the amino acid sequence of SEQ ID NO:3, or an isolated DNA complementary thereto.
 4. The DNA of claim 1, and which contains the whole of the nucleotide sequence of SEQ ID NO:4.
 5. The DNA of claim 2, which contains the whole of the nucleotide sequence of SEQ ID NO:
 5. 6. An isolated DNA which encodes a desert hedgehog protein of human origin having the nucleotide sequence of SEQ ID NO:5, or an isolated DNA complementary thereto.
 7. An isolated DNA which encodes a desert hedgehog protein of human origin having the nucleotide sequence of SEQ ID NO:6, or an isolated DNA complementary thereto.
 8. The DNA of any one of claims 4, 6, 7, 1, 2 or 3, which is inserted into an autonomously replicable vector.
 9. A transformed cell obtained by introducing the DNA of claim 8, into an appropriate host cell derived from a microbe, plant or animal.
 10. A process for producing a desert hedgehog protein of human origin, which comprises culturing the transformed cell of claim 9 to generate said desert hedgehog protein of human origin, and collecting the generated desert hedgehog protein of human origin.
 11. The process of claim 10, wherein the generated desert hedgehog protein of human origin is collected by one or more methods selected from the group consisting of salting out, dialysis, filtration, concentration, fractional precipitation, ion-exchange chromatography, gel filtration chromatography, adsorption chromatography, isoelectric focusing chromatography, hydrophobic chromatography, reversed phase chromatography, affinity chromatography, gel electro-phoresis and isoelectric focusing gel electrophoresis.
 12. The process of claim 10, wherein the generated desert hedgehog protein of human origin is collected through immunoaffinity chromatography using a monoclonal antibody that recognizes a desert hedgehog protein of human origin. 